Preformulation

Testing of
Solid Dosage Forms
Professor Dr. Narong Sarisuta
Department of Manufacturing Pharmacy
Faculty of Pharmacy, Mahidol University
Bangkok, Thailand
 Preformulation testing is the first step in the
rational development of dosage forms of a
drug substance.
 It can be defined as an investigation of physical
and chemical properties of a drug substance -
alone and when combined with excipients.
 The overall objective of preformulation testing is
to generate information useful to the formulator
in developing stable and bioavailable dosage
forms which can be mass-produced.
 During the early development of a new drug substance,
the synthetic chemist, alone or in cooperation with
specialists in other disciplines (including
preformulation), may record some data which can be
appropriately considered as preformulation data.
 This early data collection may include such information
as
- gross particle size,
- melting point,
- infrared analysis,
- thin-layer chromatographic purity,
- and other such characterizations of different
laboratory-scale batches.
 These data are useful in guiding, and becoming part of,
the main body of preformulation work.
Steps in Preformulation Process Pharmaceutical Research
1. Stability i. Solubility
a. Solid State (1) Water and Other Solvents
(1) Temperature (2) pH-Solubility Profile
(2) Light (3) Salt Forms
(3) Humidity (4) Cosolvents
b. Solution (5) Complexation
(1) Solvent (6) Prodrug
(2) pH j. Effect of pH on UV Spectra
(3) Light k. Ionization Constant
2, Solid State Compatibility l. Volatility
a. TLC Analysis m. Optical Activity
b. DRS Analysis n. Polymorphism Potential
3. Physico-chemical Properties o. Solvate Formation
a. Molecular Structure and Weight 4. Physico-mechanical Properties
b. Color a. Bulk and Tapped Density
c. Odor b. Compressibility
d. Particle size, Shape, and Crystallinity c. Photomicrograph
e. Melting Point 5. In Vitro Availability Properties
f. Thermal Analysis Profile a. Dissolution of Drug Crystal Per se
(1) DTA b. Dissolution of Pure Drug Pellet
(2) DSC c. Dissolution Analysis of Pure Drug
(3) TGA d. Rat Everted Gut Technique
g. Hygroscopicity Potential 6. Other Studies
h. Absorbance Spectra a. Plasma Protein Binding
(1) UV b. Effect of Compatible Excipients
(2) IR on Dissolution
c. Kinetic Studies of Solution
Degradation
d. Use of Radio-labeled Drug
 The formal preformulation study should start at the
point after biological screening, when a decision is
made for further development of the compound in
clinical trials.
 Before embarking upon a formal program, the
preformulation scientist must consider the following:
1. The available physicochemical data (including
chemical structure, different salts available)
2. The therapeutic class of the compound and anticipated
dose
3. The supply situation and the development schedule
(i.e., the time available)
4. The availability of a stability-indicating assay
5. The nature of the information the formulator should
have or would like to have
1. ORGANOLEPTIC PROPERTIES
1.1 Color

Unappealing to the eye ==> instrumental methods or

variable from bat
ch to batch

Record of early batches ==> establishing “specs” is

very useful for later production

Undesirable or ==> incorporation of a dye variable

color in the body or coating
1.2 Odor and Taste
Unpalatable ==> use of less soluble chemical form
(bioavailability not compromised!)

==> suppressed by - flavors

- excipients
- coating
Drug substances
irritating to skin ==> handling precautions or
sternutatory (sneezing)

Flavors, dyes, excipients used ==> stability

bioavailability
Table 1. Suggested Terminology to Describe
Organoleptic Properties of Pharmaceutical
Powders

Color Odor Taste

Off-white Pungent Acidic

Cream yellow Sulfurous Bitter
Tan Fruity Bland
Shiny Aromatic intense
Odorless Sweet
Tasteless
 2. PURITY
 Materials with impurities not necessary to be
rejected
 Another control parameter for comparison with
subsequent batches
 More direct concerns - impurity can affect:

- Stability: metal contamination in ppm

- Appearance: off-color -> recrystallized -> white
- Toxic: aromatic amine (p-amino phenol) -> carcinogenic
 Often remedial action => simple recrystallization
Cimetidine-acid hydrolysis
OH-

H+
 Techniques used for characterizing purity are the
same as used in preformulation study :
- Thin layer chromatography (TLC)
- High-pressure liquid chromatography (HPLC)
- Gas chromatography (GC)
 Impurity index (II) defined as the ratio of all
responses (peak areas) due to components other
than the main one to the total area response.
 Homogeneity index (HI) defined as the ratio of the
response (peak area) due to the main component
to the total response.
Example:
Main component - retention time: 4.39 min
- area response: 4620
Impurities - 7 minor peaks
- total area response : 251
Impurity index = 251/(4620 + 251)
= 0.0515
Homogeneity index = 1 - 0.0515
= 0.9485
 USP Impurity Index defined as a ratio of responses
due to impurities to that response due to a defined
concentration of a standard of the main component.
(using TLC)
General limit 2 % impurities
 All II, HI, USP II are not absolute measures of
impurity since the specific response (molecular
absorbances or extinction coefficient) due to each
impurity is assumed to be the same as that of the
main component.
 More accurate analysis - identification of each
individual impurity followed by preparation of
standards for each one of them.
 Other useful tools in assessment of
impurity:
- Differential Thermal Analysis (DTA)
- Thermogravimetric Analysis (TGA)
- Differential Scanning Calorimetry (DSC)
- Powder X-Ray Diffraction (PXRD)
 DSC thermograms of
pure acyclovir and
pure ethylcellulose film
s
acyclovir

Ethylcellulose film

DSC thermograms of
ethylcellulose film
containing 12.8 %
acyclovir with
15 % propylene glycol
and 10 % Tween 80
Cimetidine
3. PARTICLE SIZE, SHAPE, AND SURFACE AREA
Effects of particle size distribution and shape on:
- Chemical and physical properties of drug substances.
- Bioavailability of drug substances (griseofulvin,
chlorpropamide).
- Flow and mixing efficiency of powders and granules
in making tablets.
- Fine materials tend to require more amount of
granulating liquid (cimetidine).
- Stability, fine materials relatively more open to
attack from atmospheric O2, heat, light, humidity, and
interacting excipients than coarse materials. (Table 2)
 Table 2. Influence of Particle Size on Reaction of Sulfacetamide
with Phthalic anhydride in 1:2 Molar Compacts after 3 hr at 95 oC

Particle size of % Conversion

sulfacetamide + SD
(µ m)

128 21.54 + 2.74

164 19.43 + 3.25
214 17.25 + 2.88
302 15.69 + 7.90
387 9.34 + 4.41

Weng and Parrott

 Very fine materials are difficult to handle, overcome by
creating solid solution in a carrier (water-soluble polymer).
 Important to decide, maintain, and control a desired size
range.
 Safest - grind most new drugs with particle diameter > 100
µ m (~ 140 mesh) down to ~ 10 - 40 µ m (~ 325 mesh).
 Particles with diameter < 30 µ m (~ 400 mesh), grinding is
unnecessary except needle-like => improve flow.
 Drawbacks to grinding:
- material losses
- static charge build-up
- aggregation => increase hydrophobicity
=> lowering dissolution rate
- polymorphic or chemical transformations
3.1 General Techniques For Determining
Particle Size
3.1.1 Microscopy
- Most rapid technique.
- But for quantitative size determination requires
counting large number of particles.
- For size ~ 1 µ m upward (magnification x400).
- Suspending material in nondissolving fluid (water
or mineral oil)
- Polarizing lens to observe birefringence => change
in amorphous state after grinding?
Ketoprofen
Eudragit L100
3.1.2 Sieving
- Quantitative particle size distribution analysis.
- For size > 50 µ m upward.
- Shape has strong influence on results.
3.1.3 Electronic means
To encompass most pharmaceutical
powders ranging in size 1 - 120 µ m:
- Blockage of electrical conductivity path
(Coulter)
- Light blockage (HIAC) [adopted by USP]
- Light scattering (Royco)
- Laser scattering (Malvern)
3.1.4 Other techniques
- Centrifugation
- Air suspension
- Sedimentation (Adreasen pipet,
recording balance)
Disfavor now because of their tedious
nature.
Table 3. Common Techniques for Measuring Fine Particles of
Various Sizes

Technique Particle size (µ m)

Microscopic 1 - 100
Sieve > 50
Sedimentation >1
Elutriation 1 - 50
Centrifugal < 50
Permeability >1
Light scattering 0.5 - 50

(Parrott)
(Undersize)
(Undersize)
 3.2 Determination of Surface Area
 Surface areas of powders
-> increasing attention in recent years: reflect the particle size
 Grinding operation:
particle size ==> surface area.
 Brunauer-Emmett-Teller (BET) theory of adsorption
Most substances will adsorb a monomolecular layer of a gas
under certain conditions of partial pressure (of the gas) and
temperature.
Knowing the monolayer capacity of an adsorbent (i.e., the
quantity of adsorbate that can be accommodated as a monolayer on
the surface of a solid, the adsorbent) and the area of the adsorbate
molecule, the surface area can, in principle be calculated.
 Most commonly, nitrogen is used as the adsorbate at a specific partial
pressure established by mixing it with an inert gas, typically helium. The
adsorption process is carried out at liquid nitrogen temperature (-195 oC).
It has been demonstrated that, at a partial pressure of nitrogen
attainable when it is in a 30 % mixture with an inert gas and at -195 oC, a
monolayer is adsorbed onto most solids.
Apparently, under these conditions the polarity of nitrogen is
sufficient for van de Waals forces of attraction between the adsorbate and
the adsorbents to be manifest.
The kinetic energy present under these conditions overwhelms the
intermolecular attraction between nitrogen atoms. However, it is not
sufficient to break the bonding between the nitrogen and dissimilar atoms.
The latter are most often more polar and prone to van de Waals forces of
attraction.
The nitrogen molecule does not readily enter into chemical
combinations, and thus its binding is of a nonspecific nature (I.e., it enters
into a physical adsorption); consequently , the nitrogen molecule is well
suited for this role.
 Brunauer-Emmett-Teller (BET)
adsorption isotherm
1 = C-1 P + 1 (1)
λ (Po/P - 1) λ mC Po λ mC

λ = g of adsorbate per g of adsorbent

λ m = maximum value of that λ ratio for a monolayer

P = partial pressure of the adsorbate gas

Po = vapor pressure of the pure adsorbate gas
C = constant
P, Po, and C are temperature-dependent
 The values of λ (g of adsorbate/g of adsorbent) at
various P values (partial pressure of the adsorbate gas)
could be obtained from the experiment through
instrument.
 Po (vapor pressure of the pure adsorbate gas) can be
obtained from the literature.
 Plotting the term 1/[λ (Po/P - 1)] against P/Po will
obtain a straight line with
slope = (C - 1)/λ mC
intercept = 1/λ mC
 The term C and λ m can readily be obtained
 Dynamic Method of Gas Adsorption
 Accurately weighing the sample into an appropriate container
 Immersing the container in liquid nitrogen
 Passing the gas over the sample
 Removing the liquid nitrogen when the adsorption is complete
(as signaled by the instrument)
 Warming the sample to about the room temperature
 Measuring (via the instrument) the adsorbated gas released
(column 3 of Table 5)
 Performing the calibration by injecting known amounts of
adsorbated gas into the proper instrument port (column 4 and
5 of Table 5)
 P is the product of the fraction of N2 in the gas mixture (column
1 of Table 5) and the ambient pressure
 At relatively large diameters, the specific surface
area is insensitive to an increase in diameter
 At very small diameters the surface area is
comparatively very sensitive.
 Relatively high surface area most often reflects a
relatively small particle size, except porous or
strongly agglomerated mass
 Small particles (thus of high surface area)
agglomerate more readily, and often to render the
inner pores and surfaces inaccessible to dissolution
medium
4. SOLUBILITY
 Solubility > 1 % w/v
=> no dissolution-related absorption problem
 Highly insoluble drug administered in small doses
may exhibit good absorption
 Unstable drug in highly acidic environment of
stomach, high solubility and consequent rapid
dissolution could result in a decreased
bioavailability
 The solubility of every new drug must be
determined as a function of pH over the
physiological pH range of 1 - 8
 4.1 Determination of Solubility
4.1.1 Semiquantitative determination:

Solvent Vigorously Examine

(fixed volume) shaking visually

Adding solute in small

incremental amounts

Undissolved
solute particles ?

No Yes
“LAW OF MASS ACTION”

Estimated solubility Total amount

added up
 4.1.2 Accurately Quantitative determination:

Shaking at constant
Excess drug powder Ampul/vial temperature
150 mg/ml (15 %) (2-5 ml) (25 or 37 oC)
+ solvent 2 - 8 oC ?
The first few ml’s of the filtrates should be
discarded due to possible filter adsorption 48 hr

Determine the drug Membrane filter

concentration in the 0.45 µ m
filtrate
72 hr
Same Determine the drug Membrane filter
concentration ? concentration in the 0.45 µ m
filtrate
? hr
Solubility
Determine the drug Membrane filter
concentration in the 0.45 µ m
filtrate
 4.1.3 Unique Problems in Solubility
Determination of Poorly Soluble Compounds
 Solubilities could be overestimated due to the presence of
soluble impurities
 Saturation solubility is not reached in a reasonable length of
time unless the amount of solid used is greatly in excess of
that needed to saturation
 Many compounds in solution degrade, thus making an
accurate determination of solubility difficult
 Difficulty is also encountered in the determination of
solubility of metastable forms that transform to more stable
forms when exposed to solvents
 4.2 pH-Solubility Profile

Stir in beaker Continuous

Excess drug
with distilled stirring of
powder
water suspension

Determine the
concentration Filter Measure Stirring Add
of drug in pH of acid/base
the filtrate suspension

SOLUBILITY pH
Log aqueous solubility ( µ mol) 5

Indomethacin
4 (weak acid)

3 Chlorpromazine
(weak base)
2

1 Oxytetracycline
(amphoteric)

2 4 6 8 10 12 14

pH
 Poorly-soluble weakly-acidic drugs:

pH = pKa + log [(St - So)/So] (2)

 Poorly-soluble weakly-basic drugs:

pH = pKa + log [So/(St - So)] (3)

where
So = solubility of unionized free acid or base
St = total solubility (unionized + ionized)
 4.3 Salt Forms
NSAID’s alclofenac, diclofenac, fenbufen,
ibuprofen, naproxen
Weak acid pKa ~ 4, low solubility
Salt forms sodium
N-(2-hydroxy ethyl) piperazinium
arginium
N-methylglucosammonium
Solubility
diclofenac (free acid) : 0.8 x 10 -5 M (25 oC)
diclofenac sodium : 24.5 mg/ml (37 oC)
 4.3 Salt Forms (cont.)
Quinolones enoxacin, norfloxacin,
ciprofloxacin

Salt forms lactate, acetate, gluconate,

galacturonate, aspartate,
glutamate, etc.
Solubility
Free base : < 0.1 mg/ml (25 oC)
Salt forms : > 100 mg/ml (25 oC)
 4.4 Solubilization
Drug not an acidic or basic, or the acidic or basic character
not amendable to the formation of a stable salt
 Use more soluble metastable polymorph
 Use of complexation (eg. Ribloflavin-xanthines complex)
 Use of high-energy coprecipitates that are mixtures of solid
solutions and solid dispersions (eg. Griseofulvin in PEG 4000,
6000, and 20,000)
in PEG 4000 and 20,000 -> supersaturated solutions
in PEG 6000 -> bioavailability in human twice > micronized
drug
 Use of suitable surfactant
Cimetidine
 4.4.1 Complexation

Complexation can be analyzed and explained on the basis of

“law of mass action” as follows:
D (solid) D (solution) (4)
xD + yC DxCy (5)
St = [D] + x[DxCy] (6)
where
D = drug molecule
C = complexing agent (ligand)
St = total solubility of free drug [D] and the
drug in the complex [DxCy]
Benzocaine-caffeine complex
Ligand (Complexing Agents)
- Vitamin K - Caffeine
- Menadione - Benzoic acid
- Cholesterol - PEG series
- Cholate salt - PVP
- β -cyclodextrin
Formulation point of view:
1. How much will a specific complexing agent be used
for a certain amount of drug?
2. How does the resultant complex affect the safety,
stability, and therapeutic efficacy of the product?
 Stoichiometric ratio = moles of drug in complex
moles of complexing agent in the complex
(7)
x:y = DT - R (8)
b-a
DT = Amount of total drug added in excess (than its solubility) to the system
 5. Dissolution

kd << ka => “dissolution rate-limited”

kd ka ke
C, Vc
D Xg
Dissolution Absorption Xc Elimination

Absorption site Central compartment

(gi-tract) (blood circulation)

Diagram showing dissolution and absorption of

solid dosage form into blood circulation
5.1 Intrinsic Dissolution
5.1.1 Film Theory
The dissolution of a solid in its own solution is
adequately described by Noyes-Nernst’s “Film Theory
”
-dW = DAK (Cs - C) (9)
dt h
where
dW/dt = dissolution rate
A = surface area of the dissolving solid
D = diffusion coefficient
K = partition coefficient
h = aqueous diffusion layer
Cs = solubility of solute
C = solute concentration in the bulk medium
 5.1 Intrinsic Dissolution
5.1.1 Film Theory
The dissolution of a solid in its own solution is adequately
described by Noyes-Nernst’s “Film Theory”
Cs
- dW/dt = ADK(Cs- C)/h

dW/dt = dissolution rate of solid

A = surface area of dissolving solid D
D = diffusion coefficient
K = partition coefficient
A
Cs = solubility of solute
C = solute concentration in bulk medium
h = aqueous diffusion layer thickness h
 Intrinsic dissolution rate (mg/cm2/min) is
characteristics of each solid compound in a
given solvent under fixed hydrodynamic
conditions
 Intrinsic dissolution rate helps in predicting if
absorption would be dissolution rate-limited
 > 1 mg/cm2/min --> not likely to present
dissolution rate-limited absorption problems
 < 0.1 mg/cm2/min --> usually exhibit dissolution
rate-limited absorption
 0.1 - 1.0 mg/cm2/min --> more information is
needed before making any prediction
5.1.2 Method of Determination
5.1.2.1 Rotating-disk method (Wood apparatus)

Stirring shaft

Lower punch

Rubber gasket
Tablet die

Compressed tablet
Dissolution medium
5.1.2.2 Nelson Constant Surface Method

Dissolution
medium
Rotating
Paddle
Harden wax
or paraffin Tablet surface
 5.2 Particulate Dissolution
 Particulate dissolution is used to study the
influence on dissolution of particle size, surface
area, and mixing with excipients.
 The rate of dissolution normally increased with a
decrease in the particle size.
 Occasionally, however, an inverse relationship of
particle size to dissolution is encountered.
 This may be explained on the basis of effective or
available, rather than absolute, surface area; and it
is caused by incomplete wetting of the powder.
 Incorporation of a surfactant in the dissolution
medium may provide the expected relationship.
5.2.1 Effect of particle size of phenacetin on
dissolution rate of the drug from granules

0.11 - 0.15 mm
Amount Dissolved (mg in 500 ml)

0.15 - 0.21 mm

0.21 - 0.30 mm
0.30 - 0.50 mm

0.50 - 0.71 mm

Time (min)
(Finholt)
5.2.2 Means of enhancing the slow
dissolution:
in absence of more soluble physical or chemical
form of the drug -
 Particle size reduction (most commonly used).
 Enhanced surface area by adsorbing the drug
on an inert excipient with a high surface area,
i.e., fumed silicon dioxide.
 Comelting, coprecipitating, or triturating the
drug with some excipients.
 Incorporation of suitable surfactant.
 5.3 Prediction of Dissolution Rate
Consider the dissolution of 22 mg of 60/80 mesh
hydrocortisone in 500 ml of water. The aqueous solubility
of hydrocortisone is 0.28 mg/ml. The 60/80 mesh fraction
corresponds to 212 µ m or 2.12x10-2 cm in diameter. The
density of hydrocortisone is 1.25 g/ml. The volume of a
sphere is (4/3)π r3. Assuming that all particles are spheres
of the same diameter, 22 mg would correspond to

22 x 10-3 3 = 3,500 spherical particles

1.25 4π x (1.06)3 x 10-6

The area of a sphere is given by 4π r2. Therefore, the area

of 3,500 particles of average radius 1.06x10-2 cm is
4π x (1.06)2 x 10-4 x 3,500 = 4.94 cm2
The dissolution rate according to Eq.(9) is

-dW = DAK (Cs - C) (9)

dt h
where
D = 9.0x10-6 cm2/sec (good approximation for most drugs)
A = 4.94 cm2
K = 1.0
h = 5.0x10-3 cm (diffusion layer thickness at 50 rpm stirring)
Cs = 0.28 mg/ml
C = 0 (early phase of dissolution)
Thus, for the sample of hydrocortisone,

Initial dissolution rate = 4.94 x 9.0x10-6 x 0.28

5.0x10-3
= 2.49x10-3 mg/sec
6. Parameter Affecting Absorption
The absorption of drugs administered
orally as solids consists of 2 consecutive
processes:
1. The process of dissolution, followed by
2. The transport of the dissolved materials
across gi membranes into systemic
circulation
The rate-determining step in the overall
absorption process:
For relatively insoluble compounds
-> rate of dissolution
(can be altered via physical intervention)
For relatively soluble compounds
-> rate of permeation across biological
membrane
(is dependent on size, relative aqueous and
lipid solubilities, and ionic charge of the solute
molecules)
(can be altered, in the majority of cases,
only through molecular modification)
 In making a judgement concerning the
absorption potential of a new drug
entity, the preformulation scientist
must undertake studies to delineate its
dissolution as well as permeation
behavior.
 Characterization of the permeation behavior of a new
drug must be performed at an early stage of drug
development-primarily to help avoid mistaken efforts
to improve its absorption by improving dissolution,
when in reality the absorption is permeability-limited.
 Permeability studies are of even greater
importance when analogs of the compound
having similar pharmacological attributes are
available
 Permeability studies then would aid in the
selection of the compound with the greatest
absorption potential.
6.1 Partition Coefficient
 Like biological membrane in general, the gi
membranes are largely lipoidal in character.
 The rate and extent of absorption decreased
with the increasing polarity of molecules.
 Partition coefficient (distribution coefficient):
the ratio in which a solute distributes itself
between the two phases of two immiscible
liquids that are in contact with each other
(mostly n-octanol/water).
Comparison Between Colonic Absorption and Lipid/Water
Partition of the Un-ionized forms of Barbiturates

Chloroform/water
Barbiturate % Absorbed partition coefficient

Barbital 12 + 2 0.7
Aprobarbital17 + 2 4.0
Phenobarbital 20 + 3 4.8
Allylbarbituric acid23 +3 10.5
Butethal 24 + 3 11.7
Cyclobarbital 24 + 3 18.0
Pentobarbital 30 + 2 23.0
Secobarbital40 + 3 50.7
Hexethal 44 + 3 > 100.0
(Schanker)
 6.2 Ionization Constant
 The unionized species are more lipid-soluble
and hence more readily absorbed.
 The gi absorption of weakly acidic or basic
drugs is related to the fraction of unionized dru
g in solution.
 Factors affecting absorption:

- pH at the site of absorption

- Ionization constant
- Lipid solubility of unionized species
“pH-partition theory”
Henderson-Hasselbalch equation
For acids:
pH = pKa + log [ionized form]/[unionized form]
For bases:
pH = pKa + log [unionized form]/[ionized form]

Determination of Ionization Constant

1. Potentiometric pH-Titration
2. pH-Spectrophotometry Method
3. pH-Solubility Analysis